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巨大芽孢杆菌中参与预钴胺素-2脱氢及金属离子插入以合成西罗血红素和钴胺素过程所需酶的鉴定与功能分析。

Identification and functional analysis of enzymes required for precorrin-2 dehydrogenation and metal ion insertion in the biosynthesis of sirohaem and cobalamin in Bacillus megaterium.

作者信息

Raux Evelyne, Leech Helen K, Beck Richard, Schubert Heidi L, Santander Patricio J, Roessner Charles A, Scott A Ian, Martens Jan H, Jahn Dieter, Thermes Claude, Rambach Alain, Warren Martin J

机构信息

School of Biological Sciences, Queen Mary, University of London, Mile End Road, London E1 4NS, UK.

出版信息

Biochem J. 2003 Mar 1;370(Pt 2):505-16. doi: 10.1042/BJ20021443.

Abstract

In Bacillus megaterium, the hemAXBCDL genes were isolated and were found to be highly similar to the genes from Bacillus subtilis that are required for the conversion of glutamyl-tRNA into uroporphyrinogen III. Overproduction and purification of HemC (porphobilinogen deaminase) and -D (uroporphyrinogen III synthase) allowed these enzymes to be used for the in vitro synthesis of uroporphyrinogen III from porphobilinogen. A second smaller cluster of three genes (termed sirABC) was also isolated and found to encode the enzymes that catalyse the transformation of uroporphyrinogen III into sirohaem on the basis of their ability to complement a defined Escherichia coli (cysG) mutant. The functions of SirC and -B were investigated by direct enzyme assay, where SirC was found to act as a precorrin-2 dehydrogenase, generating sirohydrochlorin, and SirB was found to act as a ferrochelatase responsible for the final step in sirohaem synthesis. CbiX, a protein found encoded within the main B. megaterium cobalamin biosynthetic operon, shares a high degree of similarity with SirB and acts as the cobaltochelatase associated with cobalamin biosynthesis by inserting cobalt into sirohydrochlorin. CbiX contains an unusual histidine-rich region in the C-terminal portion of the protein, which was not found to be essential in the chelation process. Sequence alignments suggest that SirB and CbiX share a similar active site to the cobaltochelatase, CbiK, from Salmonella enterica.

摘要

在巨大芽孢杆菌中,hemAXBCDL基因被分离出来,发现它们与枯草芽孢杆菌中那些将谷氨酰 - tRNA转化为尿卟啉原III所需的基因高度相似。HemC(胆色素原脱氨酶)和 - D(尿卟啉原III合酶)的过量表达和纯化使得这些酶可用于从胆色素原体外合成尿卟啉原III。还分离出了另一个由三个基因组成的较小基因簇(称为sirABC),并发现它们编码的酶能够互补特定的大肠杆菌(cysG)突变体,从而催化尿卟啉原III转化为 siro 血红素。通过直接酶活性测定研究了SirC和 - B的功能,发现SirC作为前咕啉 - 2脱氢酶,生成 siro 氢氯化物,而SirB作为亚铁螯合酶负责 siro 血红素合成的最后一步。CbiX是在巨大芽孢杆菌主要钴胺素生物合成操纵子中发现的一种蛋白质,与SirB具有高度相似性,并通过将钴插入 siro 氢氯化物中作为与钴胺素生物合成相关的钴螯合酶发挥作用。CbiX在蛋白质的C末端部分含有一个不寻常的富含组氨酸的区域,该区域在螯合过程中并非必需。序列比对表明,SirB和CbiX与来自肠炎沙门氏菌的钴螯合酶CbiK具有相似的活性位点。

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